CONTAMINATION OF SURFACES AND EQUIPMENT IN THE SLAUGHTERHOUSE WIHT LISTERIA MONOCYTOGENES

Snežana Ivanović; Milenko Žutić; Oliver Radinović

doi:10.46784/e-avm.v2i2.217

Archives of Veterinary Medicine (Dec 2009)

CONTAMINATION OF SURFACES AND EQUIPMENT IN THE SLAUGHTERHOUSE WIHT LISTERIA MONOCYTOGENES

Snežana Ivanović,
Milenko Žutić,
Oliver Radinović

Affiliations

Snežana Ivanović: Scientific Veterinary Institute of Serbia, Belgrade, Republic Serbia
Milenko Žutić: Scientific Veterinary Institute of Serbia, Belgrade, Republic Serbia
Oliver Radinović: Scientific Veterinary Institute of Serbia, Belgrade, Republic Serbia

DOI: https://doi.org/10.46784/e-avm.v2i2.217
Journal volume & issue: Vol. 2, no. 2

Abstract

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Listeriosis is an infective disease of many animals and humans (zoonosis). Clinically it is manifested in various forms, mostly as abortion and meningitis. The cause is Listeria monocytognes. It is an ubiquitar bacteri, found in over than 40 mam mals, 20 bird species, several fish species and insects. After infection, clinical symptoms are some times not diagnosed and the animals arrive in slaughter house as healthy animals (unapparent infection). When animals, in this case goats, arrive for slaughter, the cause of the disease can be transmitted on the equipment and possibly on meat. In our examination, immediately after slaughter of clinically healthy goats, 20 swabs were taken from the bottom of trolleys for placing of the organs, 5 swabs from knives (between glade and grip) and 20 swabs from the floor. Three days af ter slaughter, 10 swabs were taken again from floor (from ten different places) and from the bottom of trollies (20 swabs) where the intestine and uterus were placed. The swabs were incubated in selective, enriched broth refrigerated at 5-8°C. On the third and seventh day they were inoculated on blood agar (5% sheep blood), Columbia (Himedia) and MacConkey agar (Biomedics) and incubated under the temperature of 37°C for 24-48 hours. the suspect colonies from blood and Columbia agar were controlled microscopically and, because of getting pure culture, re-cultivated on the same media. For examination of biochemical activity, commercial tests were used. For the identification BBL Crys tal G/P ID kit was used. Listeria monocytogenes was iso lated from two floor swabs, one knife swab and from two swabs from trollies. Except the one from floor, each isolate of Listeria monocytogenes was isolated from the broth inoculated for seven days. Listeria monocytogenes was iso lated from two floor swabs three days after slaughter. These isolates were isolated from the broth inoculated for seven days. Our finding shows the possibility of in direct transmission of Listeria monocytogenes on meat.

Published in Archives of Veterinary Medicine

ISSN: 1820-9955 (Print); 2683-4138 (Online)
Publisher: Scientific Veterinary Institute “Novi Sad”
Country of publisher: Serbia
LCC subjects: Agriculture: Animal culture: Veterinary medicine
Website: https://niv.ns.ac.rs/e-avm/index.php/e-avm

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